Pharmaceutical composition containing para-aminobenzoic acid-N-L-rhamnoside as an active ingredient

ABSTRACT

Disclosed is a pharmaceutical composition containing p-aminobenzoic acid-N-L-rhamonoside or a pharmaceutically acceptable salt thereof as an active ingredient.

CROSS-REFERENCE TO RELATED APPLICATION

This application is a continuation-in-part of our copending application, Ser. No. 289,226 filed Aug. 3, 1981, which is a divisional application of our copending application, Ser. No. 102535 filed Dec. 11, 1979, now U.S. Pat. No. 4,313,939, which is a continuation-in-part of our application, Ser. No. 39218, filed May 15, 1979, now abandoned.

SUMMARY OF THE INVENTION

In a first aspect of the invention, there is provided a pharmaceutical composition in dosage unit form which comprises a dosage of p-aminobenzoate-N-D-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of a tumor growth.

In a second aspect of the invention, there is provided a pharmaceutical composition in oral or perenteral dosage unit form which comprises a dosage of p-aminobenzoate-N-D-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of a tumor growth.

In a third aspect of the invention, there is provided a pharmaceutical composition in dosage unit form which comprises a dosage of p-aminobenzoate-N-D-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of hyperglycemia, hyperlipemia, inflammatory diseases, pains due to the accentuation of central nerve or pyrexia due to the accentuation of central nerve.

BACKGROUND OF THE INVENTION

The present invention relates to a pharmaceutical composition containing a compound represented by the following general formula: ##STR1## wherein ¹ R denotes the residual group formed by removing the OH group of 1 position from rhamnose, or its pharmaceutically acceptable salt selected from the group consisting of its Na, K, Mg, Ca and Al salts.

The inventors of the present invention, during the course of searching chemical compounds having antitumor activity, have found that chemical compounds represented by the above-mentioned formula (1) have a number of physiological activities such as blood sugar-reducing activity, antihypertensive activity, blood lipid-reducing activity, antiinflammatory activity and central nerve-depressing activity in addition to its antitumor activity.

Although the above-mentioned aminobenzoic acid derivatives are known compounds, no report has been found on the physiological activity of the compounds.

"Inoue, et al. N-Glycosides. XIX. Preparation of anthranilic acid N-glycosides., Chemical Abstracts, Vol. 48 (1954), Column 2001 i." and "Inoue, et al. N-Glycosides. XXV. Paper chromatography of N-glycosides., Chemical Abstracts, Vol. 48 (1954), Column 2003 a." disclose the chemical syntheses of the compounds which are the active ingredients of the pharmaceutical composition of the present invention. However, there is no utility disclosed in this prior arts and no teaching of pharmaceutical "dosage unit forms".

Furthermore, although U.S. Pat. No. 2,659,689 discloses a p-aldimino benzoic ester and a composition for protecting the human skin from erythema producing rals, the composition comprising a solution of p-aldimino benzoic ester, there is no teaching of pharmaceutical "dosage unit forms".

BRIEF DESCRIPTION OF THE DRAWING

The annexed FIGS. 1 to 2 show respectively the infrared absorption spectra of respective compound No. 1 to No. 2 in Table 1.

DETAILED DESCRIPTION OF THE INVENTION

The present invention relates to a pharmaceutical composition in dosage unit form which comprises a dosage of p-aminobenzoate-N-D-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of a tumor growth, hyperglycemia, hyperlipemia, inflammatory diseases, pains due to the accentuation of central nerve or pyrexia due to the accentuation of central nerve.

The active ingredient of the pharmaceutical composition of the present invention is a compound represented by the following formula: ##STR2## wherein ¹ R is as described above, or its pharmaceutically acceptable salt selected from the group consisting of its Na, K, Mg, Ca and Al salts. The sugar moiety of the active ingredient has a structure of a pyranose ring.

The method of preparation of the active ingredient of the present invention is illustrated as follows:

A mixture of 4.5 to 5 g of p-amiobenzoic acid, 5-6 g of L-rhamnose and 0.1 to 0.5 g of ammonium chloride was heated in 40 to 90 ml of 95 to 100% ethanol or pure methanol under a reflux condenser to induce condensation. After the reaction is over, the reactant is left at room temperature or in a cool place and the crystals separated out are collected by filtering the reactant solution. These crystals are washed with water, ethanol or ethyl ether, and then recrystallized from an aqueous solution of methanol or ethanol.

In order to substitute the hydrogen atom of the carboxyl group of the thus prepared compound with a base, it is preferable to follow the known method. The compound, paraaminobenzoic acid-N-L-rhamnoside, is dissolved in an aqueous ethanolic solution and an inorganic salt is added to the solution to effect the substitution.

The physical properties of the compounds (the active ingredient of the pharmaceutical composition of the present invention) prepared by the above-mentioned methods are shown in Table 1, and their infrared absorption spectra are respectively shown in FIGS. 1 to 2. Methods of determination of the physical properties are as follows.

                                      TABLE 1                                      __________________________________________________________________________     Physical properties of the active ingredients                                                                 Ultraviolet                                                Melting                                                                              Specific                                                                              Elementary                                                                            absorption                                                 point rotation                                                                              analysis (%)                                                                          Maximum                                         Compound   (°C.)                                                                         .sup.[α] D.sup.20                                                               C:H:N  (millimicron)                                   __________________________________________________________________________       p-aminobenzoic                                                                          169-170                                                                              -28.6 in                                                                              55.0:6.2:4.8                                                                          290, 220                                          acid-N--L-                                                                              (decomp.)                                                                            94% ethanol                                                                           (55.1:6.0:4.9)                                           rhamnoside                                                                     Sodium p-amino-                                                                         173-178                                                                              +80    51.0:5.1:4.8                                                                          273                                               benzoate-N--L-                                                                          (decomp.)                                                                            in water                                                                              (51.1:5.2:4.6)                                           rhamnoside                                                                   __________________________________________________________________________      Note:                                                                          (: : ) = theoretical values of C, H and N (%).                           

(1) Melting point: determined by the use of micro melting point determination apparatus made by Yanagimoto Works, Japan.

(2) Specific rotation: determined by using direct-reading polarimeter Model OR-50 made by Yanagimoto Works, Japan, with a thickness of 50 mm of an aqueous ethanolic solution of the acidic active ingredient and an aqueous solution of the sodium salt of the acidic active ingredient.

(3) Molecular composition: Elementary analysis was carried out by using CHN-Coder Model MT-2 made by Yanagimoto Works, Japan.

(4) Ultraviolet absorption spectrum: by using self-recording spectrophotometer Model PS-3T made by Hitachi Works, Japan, on an aqueous ethanolic solution of the acidic active ingredient and on an aqueous solution of the sodium salt of the acidic active ingredient.

(5) Infrared absorption spectrum: determined by KBr-method using infrared absorption spectrometer Model DS-701G made by Nippon Bunko Co., Ltd., Japan. The chart number of the spectrogram coincides with the number of specimens of the active ingredient.

The followings are the physiological properties of the active ingredient of the pharmaceutical composition of the present invention described in the order of (1) acute toxicity, (2) antimicrobial activity, (3) mutagenicity, (4) delayed-type intracutaneous reaction and (5) antibody-producing activity.

(1) Acute toxicity:

Acute toxicity of the active ingredients was examined by respective intraperitoneal and oral (forcible) administration to ICR-JCL mice. The specimen was dissolved in the physiological saline solution in intraperitoneal administration, and dissolved in distilled water in oral administration.

Their symptoms were observed after administration until the 7th day of administration, and LD₅₀ of the specimen was obtained from the mortality accumulated to the 7th day, according to the graphic method of Litchfield-Wilcoxon. The result is shown in Table 2. As is seen in Table 2, the active ingredient is qualified to be highly safe active ingredient of the pharmaceutical composition, having LD₅₀ more than 10 g/kg, regardless of the route of administration.

                  TABLE 2                                                          ______________________________________                                         Acute toxicity of the active ingredient                                                        LD.sub.50 in g/kg                                                              Route of administration                                        Compound          Intraperitoneal                                                                            Oral                                             ______________________________________                                         Sodium p-aminobenzoate-                                                                          15.00       12.80                                            N--L-rhamnoside                                                                ______________________________________                                    

(2) Anti-microbial activity:

The active ingredient was dissolved in distilled water at a series of two fold dilution system. These diluted solutions were mixed with agar medium in 9 times by volume and the mixture was poured into a petridish. Heart infusion agar medium was used for bacteria, and Sabouraud's agar medium was used for fungi. After streaking with the preculture, the inoculated plates were incubated at 37° C. for 20 to 24 hours for bacteria and at 25° C. for 3 to 7 days for fungi, and then the growth was examined. The following microorganisms were used for assessing the antimicrobial activity:

Pseudomonas aeruginosa IAM 1514

Escherchia coli IFO 12734

Staphylococcus aureus 209 P

Bacillus subtilis IAM 1069

Saccharomayces cerevisiae IAM 4207

Candida albicans ATCC 752

Trichophyton mentagrophytes IFO 6124

Aspergillus niger IAM 3001

As the result of the above-mentioned tests, it was found that the active ingredient did not show any growth inhibition against all the microorganisms, at a concentration of 1 mg/ml.

(3) Mutagenicity:

As the first stage, the active ingredient was tested by rec-assay (i), and as the second stage, it was tested by reversion assay (ii).

(i) A strain of Bacillus subtilis M 45, a defectant of recombination repair, and a wild strain of Bacillus subtilis H 17 keeping recombination repair activity were inoculated to make their own streaks not crossed at the start on a B-2 agar culture plate (made by dissolving 10 g of meat extract, 10 g of polypeptone, 5 g of sodium chloride and 15 g of agar in 1000 ml of distilled water at a pH of 7.0). Then, a circular sheet of filter paper 8 mm in diameter, which absorbed 0.04 ml of an aqueous solution of the active ingredient (using sterilized water) was put on the surface of the agar plate so as to cover the starting point of the above-mentioned streaks of bacterial culture. The inoculated B-2 agar culture was kept at 37° C. for a night and the length of growth-inhibited region was measured. Kanamycin was used as the negative control and Mitomycin C was used as the positive control. The results of the rec-assay are shown in Table 3.

(ii) The strains TA 98 and TA 100 (both are histidine requiring) of Salmonella typhimurium were used in the reversion assay.

Into 2 ml of a soft agar culture medium (the medium itself contains 6 g of sodium chloride and 6 g of agar in 1000 ml of distilled water) to which one tenth by volume of an aqueous solution of 0.5 mM of biotin and 0.5 mM of histidine had been added, 0.1 ml of the bacterial suspension and 0.1 ml of an aqueous solution of the active ingredient were admixed and the mixture was layered on the minimum agar culture medium. After 2 days of incubation at 37° C., the number of revertant colonies was counted. Furylfuramide (AF-2) was used as the positive control. The results of the reversion assay are shown in Table 4.

As is seen in Table 3, the active ingredient did not show any mutagenicity at a high concentration of 5000 microgram/disk. And as is seen in Table 4, the rate of occurrence of mutation by the active ingredient of the pharmaceutical composition of the present invention did not show any difference from that in the control to which no substance was added, even at a high concentration of 5000 microgram/plate. These findings demonstrate that the active ingredient is safe in view of mutagenicity.

                  TABLE 3                                                          ______________________________________                                         Result of rec-assay                                                                                Length of growth-                                                       Concen-                                                                               inhibition zone                                                                             *Dif-                                                        tration  H 45     H 17  ference                                 Compound       (μg/disk)                                                                            (mm)     (mm)  (mm)                                    ______________________________________                                         Sodium p-aminobenzoate-                                                                       500      0        0     0                                       N--L-rhamnoside                                                                               5,000    0        0     0                                       Kanamycin       10      5        4     1                                       Mitomycin C    0.05     12       2     10                                      ______________________________________                                          Note:                                                                          *Difference = length of inhibition zone of M 45 minus length of inhibitio      zone of H 17.                                                            

                  TABLE 4                                                          ______________________________________                                         Result of reversion assay                                                                            Number of revertant                                                  Concentration                                                                            colonies (n/plate)                                       Compound      (μg/plate)                                                                              TA 100    TA 98                                      ______________________________________                                         Sodium p-aminobenzo-                                                                         5,000        73        4                                         N--L-rhamnoside                                                                Furylfuramide 0.1         911       167                                        Control (nothing added)                                                                      --          149        13                                        ______________________________________                                    

(4) Delayed-type intracutaneous reaction:

In order to know the effects of the active ingredient on cellular immunity, the food pad reaction test was carried out using ICR-JCL mice as experimental animals and erythrocytes of sheep as an antigen.

A mouse was primary-sensitized by injecting 0.2 ml of 10% suspension of sheep erythrocytes in physiological saline solution from the caudal vein and after 7 days of the first sensitization, 0.05 ml of 40% suspension of sheep erythrocytes in physiological saline solution was injected in the foot pad for the second sensitization. The thickness of the foot pad was determined on the next day. The administration of the active ingredient of the pharmaceutical composition of the present invention was carried out at the dosage of 250 mg/kg/day once a day for consecutive 5 days centering around the day when the first sensitization was carried out.

As the result, the increment of the thickness of the foot pad of the mouse administered with the active ingredient showed no significant difference as compared to the increment in the group of mouse not administered with the active ingredient.

(5) Antibody-producing activity:

In order to know the effects of the active ingredient on humoral immunity, the hemagglutination test was carried out using ICR-JCL mice sensitized with sheep erythrocytes.

A mouse was sensitized by injecting 0.2 ml of 10% suspension of sheep erythrocytes in physiological saline solution from the caudal vein and after 7 days of sensitization the mouse blood was sampled for the hemagglutination test of determination of the autibody-producing activity. The active ingredient was administered for consecutive 5 days centering around the day of sensitization, intraperitoneally at the dosage of 250 mg/kg/day.

As the result, there was no significant difference in agglutination titer between the group administered with the active ingredient and the control group.

The followings are the pharmacological properties of the active ingredient of the pharmaceutical composition of the present invention described in the order of (1) blood sugar-reducing activity, (2) antihypertensive activity, (3) anti-tumour activity, (4) analgetic activity, (5) antipyretic activity, (6) antiinflammatory activity and (7) blood lipid reducing activity.

(1) Blood sugar-reducing activity:

Streptozotocin was administered intraperitoneally to a group of Wistar rats at a dosage of 60 mg/kg and after confirming the positivity of urinary sugar of the animals on the 8th day, regular insulin was further administered to the rats to reduce both the urinary sugar and the blood sugar. Out of thus treated animals, those which certainly showed a higher urinary sugar value and also a higher blood sugar value after a few days of insulin-administration were used as the model animals suffering from artificial diabetes mellitus. The active ingredient was administered to the model animals orally as a solution in distilled water at the respective dosages of 30 and 300 mg/kg. Blood specimens were collected after 3 and 6 hours of the administration, and the determination of glucose in the specimen was carried out by using a RaBA-kit (made by Chugai Pharmaceutical Co., Japan) according to the enzyme method.

The results are shown in Table 5. As seen in Table 5, the difference between the values of blood sugar before and after the administration of the active ingredient (Δ value) was conspicuously larger than Δ value of control.

                  TABLE 5                                                          ______________________________________                                         Blood sugar-reducing activity                                                                        Change (Δ value)                                                         (mg/dl) of blood                                                      Dose     sugar after                                              Compound       (mg/kg)    3 hrs.   6 hrs.                                      ______________________________________                                         Sodium p-aminobenzoate-                                                                        30        -157     -151                                        N--L-rhamnoside                                                                               300        -115     -121                                        Control        --          -36      -39                                        ______________________________________                                    

(2) Antitumour activity (I):

Sarcoma-180 were transplanted subcutaneously into the right axillary of ICR-JCL mice at the rate of 1×10⁶ cells/mouse, and from after 24 hours of transplantation an aqueous solution of the active ingredient in sterilized physiological saline solution was orally administered every other day at a dose rate of 500 mg/kg, 10 times in all. On the 25th day of the transplantation, the modular tumour(s) was extirpated and weighed.

The inhibition ratio (I.R.) (%) of the active ingredient was calculated by the following formula:

    (1-T/C)×100=I.R. (%)

wherein

T: mean weight of the tumour(s) in treated group of mice

C: mean weight of the tumour(s) in control group* of mice

The result of the test is shown in Table 6. As seen in Table 6, the active ingredient exhibited an antitumour activity.

                  TABLE 6                                                          ______________________________________                                         Antitumour activity against Sarcoma-180                                                            Inhibition ratio                                           Compound            (I.R. %)                                                   ______________________________________                                         Sodium p-aminobenzoate-N--L-                                                                       72.5                                                       rhamnoside                                                                     ______________________________________                                          Note: Amount of administration was 10 × 500 mg/kg p.o.             

Antitumour activity (II):

Lewis lung Ca. (the 3 millimeter square), were transplanted subcutaneously into the dorsum of BDF1 mice, and from from after 24 hours of transplantation an aqueous solution of sodium p-aminobenzoate-N-L-rhamnoside as active ingredient in sterilized physiological saline solution was (1) orally administered every day at the following dose rate, 20 times in all, or (2) intra-peritoneally administered every other day at the following dose rate, 10 times in all. On the 25th day of the transplantation, the nodular tumour(s) was extirpated and weighed.

The inhibition ratio (I.R.) (%) of the active ingredient was calculated by the following formula:

    (1-T/C)×100=I.R. (%)

wherein

T: mean weight of the tumour(s) in treated group of mice

C: mean weight of the tumour(s) in control group* of mice

The result of the test is shown in Table 7. As seen in Table 7, the active ingredient exhibited an antitumour activity.

                  TABLE 7                                                          ______________________________________                                         Antitumour activity against Lewis lung Ca.                                                  Dosage   Inhibition ratio                                                      (mg/kg/time)                                                                            (I.R. %)                                                 ______________________________________                                         Oral administration                                                                           400        59.0                                                                300        61.9                                                                100        53.9                                                                50         45.1                                                                10         40.1                                                 Intra-peritoneal                                                                              150        61.5                                                 administration 100        64.0                                                                50         53.1                                                                10         49.3                                                                1          49.1                                                                0.1        41.3                                                 ______________________________________                                    

(3) Analgetic activity:

Determination by the mechanical stimulation method (by applying pressure):

Female ICR mice which showed a threshold value of pain of 50 to 80 mmHg when their tail base part was pressed by a pressure stimulation apparatus (made by Natsume Works, Japan) of Takagi and Kameyama were chosen at test animals, ten animals comprising a group.

After administering the active ingredient, the test was carried out as the time passes and the applied pressure and the time period until the animal showed a quasi-escaping reaction were determined to evaluate the analgetic activity of the active ingredient.

The result is shown in Table 8. As seen in Table 8, the pressure applied on animals when the animal showed the quasi-escaping reaction was higher in animals to which the active ingredient had been applied than in animals not administered, and the time period from the beginning to the time point when the animal showed the reaction was longer in animals administered with the active ingredient than in animals not administered. Thus, the analgetic activity of the active ingredient was confirmed.

Determination by the chemical stimulation method:

The active ingredient was orally administered to a group (ten animals) of female ICR mice of age of 5 to 6 weeks, and after 30 min of the administration an aqueous 0.6% acetic acid solution was intraperitoneally injected into the mouse at a dose rate of 0.1 ml/10 g of body weight. The number of writhing syndrom which occurred in the mouse during 10 minutes after 10 minutes of intraperitoneal administration was recorded. The analgetic activity was evaluated from the writhing syndrome inhibiting ratio obtained by the following formula:

    (1-T/C)×100=writhing syndrome-inhibiting ratio (%)

wherein

T: mean number of writhing syndrome in the group administered.

C: mean number of writhing syndrome in the control group.

The result is shown in Table 9. As seen in Table 9, the active ingredient of the pharmaceutical composition of the present invention showed analgetic activity. The above-mentioned process was carried out following the method of Kostet et al. (1959).

                  TABLE 8                                                          ______________________________________                                         Analgetic activity by the mechanical stimulation method                                        Quasi-escape reaction                                                          pressure at time until                                                         (mm Hg) (sec)                                                  Compound          occurrence                                                   ______________________________________                                         Sodium p-aminobenzoate-                                                                          92        42                                                 N--L-rhamnoside                                                                Control           70        33                                                 ______________________________________                                          Note: Amount of administration, 1000 mg/kg p.o.                          

                  TABLE 9                                                          ______________________________________                                         Analgetic activity by the chemical stimulation method                          Compound                 I.R. (%)                                              ______________________________________                                         Sodium p-aminobenzoate-N--L-rhamnoside                                                                  75.0                                                  ______________________________________                                          Note: Amount of administration was 1000 mg/kg p.o.                       

(5) Antipyretic activity:

Following the method of Winter et al. (1961), a 20% suspension of beer yeast was subcutaneously injected to a group (consisting of 6 animals) of rats, and after 10 hours of fasting, the active ingredient was orally administered to the rats and their rectal temperature was determined.

The antipyretic activity is expressed by the ratio of inhibiting pyrexia due to beer yeast (I.R. %) at the time when the antipyretic activity of the active ingredient is at its maximum according to the following formula: ##EQU1## wherein T: mean rectal temperature of rats to which the active ingredient was administered.

C₁ : mean rectal temperature of rats injected beer yeast, without the active ingredient.

C₂ : mean rectal temperature of untreated rats (control).

The results is shown in Table 10. As seen in Table 10, the active ingredient exhibited a considerable antipyretic activity.

                  TABLE 10                                                         ______________________________________                                         Antipyretic activity                                                                            Antipyretic activity                                                           (suppressing pyrexia)                                         Compound         I.R. (%)                                                      ______________________________________                                         Sodium p-aminobenzoate-                                                                         91.4                                                          N--L-rhamnoside                                                                ______________________________________                                    

(6) Antiinflammatory activity:

(a) Carrageenin-edema inhibitory activity:

Following the method of Van Arman et al. (1963), the active ingredient was forcibly and orally administered to each rat of a group consisting of 10 animals at the dose rate of 1000 mg/kg, and after one hour of the administration 0.1 ml of 1% suspension of carrageenin in physiological saline solution was injected to their right foot pad. The volume of the foot pad was determined as time passes and the antiinflammatory activity was expressed by the ratio of inhibition of the swelling of the food pad due to carrageenin by the active ingredient, using the determined value of 1-4 hours from the injection and calculating by the following formula:

    (1-T/C)×100=I.R. (%)=antiinflammatory activity

wherein

T: mean value of volumes of foot pad in administered animals

C: mean value of volume of foot pad of control (not administered and then injected).

The result is shown in Table 11. As seen in Table 11, the ingredient showed the inhibitory activity against the edema caused by carrageenin.

(b) Antigranuloma activity:

Following the method of Winter et al. (1963), two cotton wool pellets were implanted into the skin of back of each rat of a group consisting of 6 rats at the symmetrical positions having the median line as the axis of symmetry, the weight of one pellet being 30±1 mg. Oral administration of 1000 mg/kg/day of the active ingredient was carried out for consecutive 7 days. On the 8th day, the granuloma formed in the rats was extirpated and weighed after drying. The antigranuloma activity expressed by the ratio of inhibition of the growth of the granuloma (I.R., %) was calculated in a manner as shown in (6)(a), and the result is shown in Table 11. As seen in Table 11, the active ingredient exhibited the inhibiting activity of growth of the granuloma.

(c) Antiexudation activity:

Following the method of Baris et al. (1965), a volume of air was injected subcutaneously in the back of each rat of a group consisting of 6 rats to make an air pouch, and then 0.5 ml of 1% cotton oil solution in sesame oil was injected into the pouch. The oral administration of 1000 mg/kg/day of the active ingredient was then begun to continue for 5 days. On the 6th day, the amount of exudated liquid into the pouch was determined and the antiexudation activity expressed by the ratio of inhibitory activity to exudation was calculated in a manner as shown in (6)(a). The result is shown in Table 11. As seen in Table 11, the active ingredient exhibited the antiexudation activity.

(d) Antiadjuvant arthritis activity:

Following the method of Fujiwara et al. (1971), Mycobacterium tuberculosis suspended in liquid paraffin was injected subcutaneously into the right foot pad of each rat of group consisting of 6 rats. After 14 days of the injection, rats with similar volume of the foot pad were chosen to form groups (10 animals/group), the active ingredient was orally administered daily from the 15th day for consecutive 7 days. The volume of the foot pad of rats was determined, and the antiadjuvant arthritis activity of the active ingredient was calculated as the ratio of inhibiting the swelling of the foot pad by using the formula shown in (6)(a). The result is shown in Table 11. As seen in Table 11, the active ingredient exhibited the antiadjuvant arthritis activity.

                  TABLE 11                                                         ______________________________________                                         Antiinflammatory activity                                                                              Gran-   Exuda-                                         Compound       Edema    uloma   tion  Arthritis                                ______________________________________                                         Sodium p-aminobenzoate-                                                                       21.7     22.1    16.2  35.9                                     N--L-rhamnoside                                                                ______________________________________                                          Note: Amount of administration of the active ingredient = 1000 mg/kg.    

(7) Blood lipid reducing activity:

Japanese male white rabbits were fed for about 3 months with solid feed (CR-1) containing 1% of cholesterol and those animals in which the increase of seral lipid component was confirmed were used as the model animals having experimental arteriosclerosis.

An aqueous solution of the active ingredient in distilled water was administered respectively at the dose rates of 30 and 300 mg/kg orally and after the administration, blood specimen was collected as time passes from the auricular vein and the change of total cholesterol (determined by the enzyme method), phospholipid (determined by the enzyme method) and beta-lipoprotein (determined by turbidmetry) in the serum was observed.

The results are shown in Table 12. In Table 12, the values of serum cholesterol (mean value of 550 mg/dl), of phospholipid (mean value of 320 mg/dl) and of beta-lipoprotein (mean value of 2500 mg/kg) before administration were respectively subtracted from the respective values after 3 and 6 hours of the administration, and only the differences are shown, respectively. Therefore, the minus value shows the decrease and the plus value shows the increase of the respective values due to the administration. As clearly seen in Table 12, the active ingredient exhibited the activity of reducing the lipid components as compared to control.

                                      TABLE 12                                     __________________________________________________________________________     Activity of reducing blood lipids                                                                Phospholipid                                                                           beta-Lipopro-                                                                          Cholesterol                                               Dose (mg/dl) tein (mg/dl)                                                                           (mg/dl)                                                   (mg/kg)                                                                             3 hrs.                                                                             6 hrs.                                                                             3 hrs.                                                                             6 hrs.                                                                             3 hrs.                                                                             6 hrs.                                   __________________________________________________________________________     Sodium p-aminobenzoate-                                                                      30  -49 -47 -134                                                                               -161                                                                               -50 -45                                      N--L-rhamnoside                                                                             300  -57 -51  -24                                                                               -232                                                                               -75 -70                                      Control             0 -19   0  +3  +8  +4                                      __________________________________________________________________________

Now, the formulation of the active ingredient to make the pharmaceutical composition of the present invention is described below.

In the case where the pharmaceutical composition is used as an antiinflammatory agent, it is able to use the pharmaceutical composition in the form which is convenient to obtain the effectiveness according to the kinds and the symptoms of the disease, and moreover, the active ingredient may be used as itself or may be used as mixtures combined with any diluent allowable in pharmaceutical process and with other medicines.

The pharmaceutical composition of the present invention is administered orally or parenterally and accordingly, the pharmaceutical composition of the present invention may take any form optionally for the oral or parenteral administration.

The pharmaceutical composition of the present invention may be offered as a form of unit administration. The form of the pharmaceutical composition of the present invention may be powder, granule, tablet, sugar-coated tablet, capsulated one, suppository, suspension, solution, emulsifiable concentrate, ampouled one, injection, etc. As a diluent, any one of solids, liquids and semisolids may be utilized, for instance, excipients, fillers, binders, wetting agents, disintegrating agents, surfactants, demulcents, dispersing agents, buffering agents, perfumes, preservatives, dissolution aids and solvents. Moreover, one or more than one of these adjuvants may be used in combination or in mixtures.

The pharmaceutical composition of the present invention may be formulated by any known method, and the amount of the active ingredient contained in the composition (preparation) is generally from 0.01% to 100% by weight.

The pharmaceutical composition of the present invention may be administered orally or parenterally to human or animals, however, it is preferably administered orally. Sublingual administration is included in oral administration. Parenteral administration includes subcutaneous-, intramuscular- and intravenous injection and the injection by drop method.

The dose of the pharmaceutical composition of the present invention depends upon the age, the personal difference and the state of disease, and whether the object is human or animal and accordingly, an extraordinal amount amy be administered than the following dose: Generally, for human, the oral dose is 0.1-1000 mg/kg body weight/day, preferably 1-500 mg/kg/day and the parenteral dose is 0.01-200 mg/kg/day, preferably 0.1-100 mg/kg/day divided into 1-4 parts, one part being administered in one time.

The followings are the more detailed explanation of the formulation and the production of the pharmaceutical composition of the present invention in examples.

EXAMPLE 1 (Formulation)

10 parts by weight of sodium p-aminobenzoate-N-L-rhamnoside,

15 parts by weight of (heavy) magnesium oxide and

75 parts by weight of lactose were uniformly mixed and formulated into powder or granules. The power is filled in capsules to be capsulated formulation.

EXAMPLE 2 (Formulation)

45 parts by weight of sodium p-aminobenzoate-N-L-rhamnoside,

15 parts by weight of starch,

16 parts by weight of lactose,

21 parts by weight of crystalline cellulose,

3 parts by weight of polyvinyl alcohol and

30 parts by weight of water were uniformly mixed, crushed and formulated, and then dried and shifted to be granules.

EXAMPLE 3 (Formulation)

Granules were prepared as in Example 2, and the mixture of 96 parts by weight of this granule and 4 parts by weight of calcium stearate was compression-formulated to be tablets 10 mm in diameter.

EXAMPLE 4 (Formulation)

94 parts by weight of sodium p-aminobenzoate-N-L-rhamnoside,

6 parts by weight of polyvinyl alcohol and

30 parts by weight of water were mixed and the mixture was processed as in Example 2 to be granules. To 90 parts by weight of the thus processed granules 10 parts by weight of crystalline cellulose were mixed and the mixture was compression-formulated to be tablets 8 mm in diameter. The tablets were coated with syrup, gelatine and precipitated calcium carbonate to be coated tablets.

EXAMPLE 5 (Formulation)

0.6 part by weight of sodium p-aminobenzoate-N-L-rhamnoside,

2.4 parts by weight of a non-ionic surfactant and

97 parts by weight of physiological saline solution were mixed under heating and then the mixture was sterilized to be an injection.

EXAMPLE 6 (Production of p-aminobenzoic acid-N-L-rhamnoside and its sodium salt)

A mixture of 3 g of p-aminobenzoic acid, 4 g of L-rhamnose and 0.1 g of ammonium chloride was heated in 30 ml of 94% ethanol under a reflux condenser. After the reaction was over, crystals separated out when the reaction mixture was left at room temperature. The crystals thus obtained by filtering were washed with water and an aqueous methanolic solution, and then recrystallized from 50% methanol. The recrystallized crystals were colorless needles. Yield was 30.9%.

Thus obtained p-aminobenzoic acid-N-L-rhamnoside was dissolved gradually into an aqueous 1% sodium hydroxide solution containing in total the calculated amount of sodium hydroxide and after filtering, the solution was condensed under reduced pressure. The crystals which separated out by the addition of a large excess of acetone to the condensate was dehydrated and dried. Colorless crystal of sodium salt was obtained at the yield of 100%. The total yield from p-aminobenzoic acid was 30.9%. 

What is claimed is:
 1. A pharmaceutical composition in dosage unit form which comprises a dosage of p-aminobenzoic acid-N-L-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of hyperglycemia.
 2. A pharmaceutical composition of claim 1 which is in the form of said pharmaceutically acceptable salt which is the sodium salt.
 3. A pharmaceutical composition in dosage unit form which comprises a dosage of p-aminobenzoic acid-N-L-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of hyperlipemia.
 4. A pharmaceutical composition of claim 3 which is in the form of said pharmaceutically acceptable salt which is the sodium salt.
 5. A pharmaceutical composition in dosage unit form which comprises a dosage of p-aminobenzoic acid-N-L-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of inflammatory diseases.
 6. A pharmaceutical composition of claim 5 which is in the form of said pharmaceutically acceptable salt which is the sodium salt.
 7. A pharmaceutical composition in dosage unit form which comprises a dosage of p-aminobenzoic acid-N-L-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of pains due to the accentuation of central nerve.
 8. A pharmaceutical composition of claim 7 which is in the form of said pharmaceutically acceptable salt which is the sodium salt.
 9. A pharmaceutical composition in dosage unit form which comprises a dosage of p-aminobenzoic acid-N-L-rhamnoside or pharmaceutically acceptable salt thereof effective for the treatment of pyrexia due to the accentuation of central nerve.
 10. A pharmaceutical composition of claim 9 which is in the form of said pharmaceutically acceptable salt which is the sodium salt. 